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High-resolution mapping of DNA polymerase fidelity using nucleotide imbalances and next-generation sequencing

机译:使用核苷酸失衡和下一代测序对DNA聚合酶保真度进行高分辨率定位

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摘要

DNA polymerase fidelity is affected by both intrinsic properties and environmental conditions. Current strategies for measuring DNA polymerase error rate in vitro are constrained by low error subtype sensitivity, poor scalability, and lack of flexibility in types of sequence contexts that can be tested. We have developed the Magnification via Nucleotide Imbalance Fidelity (MagNIFi) assay, a scalable next-generation sequencing assay that uses a biased deoxynucleotide pool to quantitatively shift error rates into a range where errors are frequent and hence measurement is robust, while still allowing for accurate mapping to error rates under typical conditions. This assay is compatible with a wide range of fidelity-modulating conditions, and enables high-throughput analysis of sequence context effects on base substitution and single nucleotide deletion fidelity using a built-in template library. We validate this assay by comparing to previously established fidelity metrics, and use it to investigate neighboring sequence-mediated effects on fidelity for several DNA polymerases. Through these demonstrations, we establish the MagNIFi assay for robust, high-throughput analysis of DNA polymerase fidelity.
机译:DNA聚合酶的保真度受内在特性和环境条件的影响。当前在体外测量DNA聚合酶错误率的策略受到错误亚型敏感性低,可扩展性差以及在可以测试的序列上下文类型中缺乏灵活性的限制。我们已经开发了通过核苷酸不平衡保真度(MagNIFi)测定法进行的放大,这是一种可扩展的下一代测序测定法,使用偏性脱氧核苷酸池将错误率定量地移至经常发生错误的范围内,因此测量很可靠,同时仍可确保准确度映射到典型情况下的错误率。该测定法可与各种保真度调节条件兼容,并使用内置模板库对碱基取代和单核苷酸缺失保真度的序列背景影响进行高通量分析。我们通过与以前建立的保真度指标进行比较来验证该测定,并使用它来研究邻近序列介导的几种DNA聚合酶对保真度的影响。通过这些演示,我们建立了用于DNA聚合酶保真度分析的强大,高通量分析的MagNIFi分析。

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